Your search keyword '"Engleka KA"' showing total 23 results

1. An Engineered Mouse to Identify Proliferating Cells and Their Derivatives.

Author

Jang J, Engleka KA, Liu F, Li L, Song G, Epstein JA, and Li D

Abstract

Background: Cell proliferation is a fundamental event during development, disease, and regeneration. Effectively tracking and quantifying proliferating cells and their derivatives is critical for addressing many research questions. Cell cycle expression such as for Ki67, proliferating cell nuclear antigen (PCNA), or aurora kinase B (Aurkb), or measurement of 5-bromo-2'-deoxyuridine (BrdU) or 3 H-thymidine incorporation have been widely used to assess and quantify cell proliferation. These are powerful tools for detecting actively proliferating cells, but they do not identify cell populations derived from proliferating progenitors over time., Aims: We developed a new mouse tool for lineage tracing of proliferating cells by targeting the Aurkb allele., Results: In quiescent cells or cells arrested at G1/S, little or no Aurkb mRNA is detectable. In cycling cells, Aurkb transcripts are detectable at G2 and become undetectable by telophase. These findings suggest that Aurkb transcription is restricted to proliferating cells and is tightly coupled to cell proliferation. Accordingly, we generated an Aurkb ER Cre/+ mouse by targeting a tamoxifen inducible Cre cassette into the start codon of Aurkb . We find that the Aurkb ER Cre/+ mouse faithfully labels proliferating cells in developing embryos and regenerative adult tissues such as intestine but does not label quiescent cells such as post-mitotic neurons., Conclusion: The Aurkb ER Cre/+ mouse faithfully labels proliferating cells and their derivatives in developing embryos and regenerative adult tissues. This new mouse tool provides a novel genetic tracing capability for studying tissue proliferation and regeneration., (Copyright © 2020 Jang, Engleka, Liu, Li, Song, Epstein and Li.)

Published

2020

2. Hemodynamic Forces Sculpt Developing Heart Valves through a KLF2-WNT9B Paracrine Signaling Axis.

Author

Goddard LM, Duchemin AL, Ramalingan H, Wu B, Chen M, Bamezai S, Yang J, Li L, Morley MP, Wang T, Scherrer-Crosbie M, Frank DB, Engleka KA, Jameson SC, Morrisey EE, Carroll TJ, Zhou B, Vermot J, and Kahn ML

Subjects

Animals, Cell Proliferation physiology, Kruppel-Like Factor 4, Kruppel-Like Transcription Factors metabolism, Mice, Transgenic, Organogenesis physiology, Transcription Factors genetics, Wnt Proteins metabolism, Zebrafish, Zebrafish Proteins metabolism, Endocardium metabolism, Gene Expression Regulation, Developmental genetics, Heart Valves growth & development, Hemodynamics physiology, Signal Transduction genetics

Abstract

Hemodynamic forces play an essential epigenetic role in heart valve development, but how they do so is not known. Here, we show that the shear-responsive transcription factor KLF2 is required in endocardial cells to regulate the mesenchymal cell responses that remodel cardiac cushions to mature valves. Endocardial Klf2 deficiency results in defective valve formation associated with loss of Wnt9b expression and reduced canonical WNT signaling in neighboring mesenchymal cells, a phenotype reproduced by endocardial-specific loss of Wnt9b. Studies in zebrafish embryos reveal that wnt9b expression is similarly restricted to the endocardial cells overlying the developing heart valves and is dependent upon both hemodynamic shear forces and klf2a expression. These studies identify KLF2-WNT9B signaling as a conserved molecular mechanism by which fluid forces sensed by endothelial cells direct the complex cellular process of heart valve development and suggest that congenital valve defects may arise due to subtle defects in this mechanotransduction pathway., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2017

3. Epicardial YAP/TAZ orchestrate an immunosuppressive response following myocardial infarction.

Author

Ramjee V, Li D, Manderfield LJ, Liu F, Engleka KA, Aghajanian H, Rodell CB, Lu W, Ho V, Wang T, Li L, Singh A, Cibi DM, Burdick JA, Singh MK, Jain R, and Epstein JA

Subjects

Acyltransferases, Adaptor Proteins, Signal Transducing genetics, Animals, Cardiomyopathies etiology, Cardiomyopathies genetics, Cardiomyopathies immunology, Cardiomyopathies pathology, Cell Cycle Proteins, Fibrosis, HEK293 Cells, Humans, Mice, Mice, Transgenic, Myocardial Infarction complications, Myocardial Infarction genetics, Myocardial Infarction pathology, Pericardium pathology, Phosphoproteins genetics, T-Lymphocytes, Regulatory pathology, Transcription Factors genetics, YAP-Signaling Proteins, Adaptor Proteins, Signal Transducing immunology, Immune Tolerance, Myocardial Infarction immunology, Pericardium immunology, Phosphoproteins immunology, T-Lymphocytes, Regulatory immunology, Transcription Factors immunology

Abstract

Ischemic heart disease resulting from myocardial infarction (MI) is the most prevalent form of heart disease in the United States. Post-MI cardiac remodeling is a multifaceted process that includes activation of fibroblasts and a complex immune response. T-regulatory cells (Tregs), a subset of CD4+ T cells, have been shown to suppress the innate and adaptive immune response and limit deleterious remodeling following myocardial injury. However, the mechanisms by which injured myocardium recruits suppressive immune cells remain largely unknown. Here, we have shown a role for Hippo signaling in the epicardium in suppressing the post-infarct inflammatory response through recruitment of Tregs. Mice deficient in epicardial YAP and TAZ, two core Hippo pathway effectors, developed profound post-MI pericardial inflammation and myocardial fibrosis, resulting in cardiomyopathy and death. Mutant mice exhibited fewer suppressive Tregs in the injured myocardium and decreased expression of the gene encoding IFN-γ, a known Treg inducer. Furthermore, controlled local delivery of IFN-γ following MI rescued Treg infiltration into the injured myocardium of YAP/TAZ mutants and decreased fibrosis. Collectively, these results suggest that epicardial Hippo signaling plays a key role in adaptive immune regulation during the post-MI recovery phase.

Published

2017

4. Loss of neurofibromin Ras-GAP activity enhances the formation of cardiac blood islands in murine embryos.

Author

Yzaguirre AD, Padmanabhan A, de Groh ED, Engleka KA, Li J, Speck NA, and Epstein JA

Subjects

Animals, Mice, Mutant Proteins genetics, Mutant Proteins metabolism, Mutation, Missense, Neurofibromin 1 genetics, ras GTPase-Activating Proteins genetics, Heart embryology, Hematopoiesis, Extramedullary, Myocardium pathology, Neurofibromin 1 metabolism, ras GTPase-Activating Proteins metabolism

Abstract

Type I neurofibromatosis (NF1) is caused by mutations in the NF1 gene encoding neurofibromin. Neurofibromin exhibits Ras GTPase activating protein (Ras-GAP) activity that is thought to mediate cellular functions relevant to disease phenotypes. Loss of murine Nf1 results in embryonic lethality due to heart defects, while mice with monoallelic loss of function mutations or with tissue-specific inactivation have been used to model NF1. Here, we characterize previously unappreciated phenotypes in Nf1-/- embryos, which are inhibition of hemogenic endothelial specification in the dorsal aorta, enhanced yolk sac hematopoiesis, and exuberant cardiac blood island formation. We show that a missense mutation engineered into the active site of the Ras-GAP domain is sufficient to reproduce ectopic blood island formation, cardiac defects, and overgrowth of neural crest-derived structures seen in Nf1-/-embryos. These findings demonstrate a role for Ras-GAP activity in suppressing the hemogenic potential of the heart and restricting growth of neural crest-derived tissues.

Published

2015

5. Hippo signaling is required for Notch-dependent smooth muscle differentiation of neural crest.

Author

Manderfield LJ, Aghajanian H, Engleka KA, Lim LY, Liu F, Jain R, Li L, Olson EN, and Epstein JA

Subjects

Acyltransferases, Adaptor Proteins, Signal Transducing chemistry, Adaptor Proteins, Signal Transducing metabolism, Animals, Aorta, Thoracic metabolism, Cell Cycle Proteins, DNA-Binding Proteins metabolism, Gene Deletion, HEK293 Cells, Hippo Signaling Pathway, Humans, Mesoderm metabolism, Mice, Muscle, Smooth metabolism, Phosphoproteins chemistry, Phosphoproteins metabolism, Protein Binding, Protein Structure, Tertiary, Receptors, Notch chemistry, TEA Domain Transcription Factors, Transcription Factors metabolism, Transcription, Genetic, YAP-Signaling Proteins, Cell Differentiation, Myocytes, Smooth Muscle cytology, Myocytes, Smooth Muscle metabolism, Neural Crest cytology, Protein Serine-Threonine Kinases metabolism, Receptors, Notch metabolism, Signal Transduction

Abstract

Notch signaling has well-defined roles in the assembly of arterial walls and in the development of the endothelium and smooth muscle of the vasculature. Hippo signaling regulates cellular growth in many tissues, and contributes to regulation of organ size, in addition to other functions. Here, we show that the Notch and Hippo pathways converge to regulate smooth muscle differentiation of the neural crest, which is crucial for normal development of the aortic arch arteries and cranial vasculature during embryonic development. Neural crest-specific deletion of the Hippo effectors Yap and Taz produces neural crest precursors that migrate normally, but fail to produce vascular smooth muscle, and Notch target genes such as Jagged1 fail to activate normally. We show that Yap is normally recruited to a tissue-specific Jagged1 enhancer by directly interacting with the Notch intracellular domain (NICD). The Yap-NICD complex is recruited to chromatin by the DNA-binding protein Rbp-J in a Tead-independent fashion. Thus, Hippo signaling can modulate Notch signaling outputs, and components of the Hippo and Notch pathways physically interact. Convergence of Hippo and Notch pathways by the mechanisms described here might be relevant for the function of these signaling cascades in many tissues and in diseases such as cancer., (© 2015. Published by The Company of Biologists Ltd.)

Published

2015

6. Pax3 and Hippo Signaling Coordinate Melanocyte Gene Expression in Neural Crest.

Author

Manderfield LJ, Engleka KA, Aghajanian H, Gupta M, Yang S, Li L, Baggs JE, Hogenesch JB, Olson EN, and Epstein JA

Published

2015

7. Pax3 and hippo signaling coordinate melanocyte gene expression in neural crest.

Author

Manderfield LJ, Engleka KA, Aghajanian H, Gupta M, Yang S, Li L, Baggs JE, Hogenesch JB, Olson EN, and Epstein JA

Subjects

Animals, Genes, Reporter, HEK293 Cells, Hippo Signaling Pathway, Humans, Luciferases biosynthesis, Luciferases genetics, Mice, Transgenic, PAX3 Transcription Factor, Phosphorylation, Protein Processing, Post-Translational, Protein Transport, Transcriptional Activation, Gene Expression Regulation, Developmental, Melanocytes metabolism, Neural Crest cytology, Paired Box Transcription Factors metabolism, Protein Serine-Threonine Kinases metabolism

Abstract

Loss of Pax3, a developmentally regulated transcription factor expressed in premigratory neural crest, results in severe developmental defects and embryonic lethality. Although Pax3 mutations produce profound phenotypes, the intrinsic transcriptional activation exhibited by Pax3 is surprisingly modest. We postulated the existence of transcriptional coactivators that function with Pax3 to mediate developmental functions. A high-throughput screen identified the Hippo effector proteins Taz and Yap65 as Pax3 coactivators. Synergistic coactivation of target genes by Pax3-Taz/Yap65 requires DNA binding by Pax3, is Tead independent, and is regulated by Hippo kinases Mst1 and Lats2. In vivo, Pax3 and Yap65 colocalize in the nucleus of neural crest progenitors in the dorsal neural tube. Neural crest deletion of Taz and Yap65 results in embryo-lethal neural crest defects and decreased expression of the Pax3 target gene, Mitf. These results suggest that Pax3 activity is regulated by the Hippo pathway and that Pax factors are Hippo effectors., (Copyright © 2014 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2014

8. Islet1 derivatives in the heart are of both neural crest and second heart field origin.

Author

Engleka KA, Manderfield LJ, Brust RD, Li L, Cohen A, Dymecki SM, and Epstein JA

Subjects

Animals, Biomarkers, Green Fluorescent Proteins genetics, LIM-Homeodomain Proteins genetics, Mice, Mice, Transgenic, Models, Animal, Myocardium cytology, Neural Crest cytology, Stem Cells cytology, Stem Cells metabolism, Transcription Factors genetics, Wnt1 Protein genetics, Wnt1 Protein metabolism, Cell Lineage, Heart embryology, LIM-Homeodomain Proteins metabolism, Myocardium metabolism, Neural Crest embryology, Transcription Factors metabolism

Abstract

Rationale: Islet1 (Isl1) has been proposed as a marker of cardiac progenitor cells derived from the second heart field and is utilized to identify and purify cardiac progenitors from murine and human specimens for ex vivo expansion. The use of Isl1 as a specific second heart field marker is dependent on its exclusion from other cardiac lineages such as neural crest., Objective: Determine whether Isl1 is expressed by cardiac neural crest., Methods and Results: We used an intersectional fate-mapping system using the RC::FrePe allele, which reports dual Flpe and Cre recombination. Combining Isl1(Cre/+), a SHF driver, and Wnt1::Flpe, a neural crest driver, with Rc::FrePe reveals that some Isl1 derivatives in the cardiac outflow tract derive from Wnt1-expressing neural crest progenitors. In contrast, no overlap was observed between Wnt1-derived neural crest and an alternative second heart field driver, Mef2c-AHF-Cre., Conclusions: Isl1 is not restricted to second heart field progenitors in the developing heart but also labels cardiac neural crest. The intersection of Isl1 and Wnt1 lineages within the heart provides a caveat to using Isl1 as an exclusive second heart field cardiac progenitor marker and suggests that some Isl1-expressing progenitor cells derived from embryos, embryonic stem cultures, or induced pluripotent stem cultures may be of neural crest lineage.

Published

2012

9. Notch activation of Jagged1 contributes to the assembly of the arterial wall.

Author

Manderfield LJ, High FA, Engleka KA, Liu F, Li L, Rentschler S, and Epstein JA

Subjects

Animals, Aorta, Thoracic, Calcium-Binding Proteins genetics, Cell Differentiation, Conserved Sequence, Intercellular Signaling Peptides and Proteins genetics, Jagged-1 Protein, Membrane Proteins genetics, Mice, Muscle, Smooth, Vascular metabolism, Neural Crest cytology, RNA, Messenger, Serrate-Jagged Proteins, Arteries growth & development, Calcium-Binding Proteins metabolism, Intercellular Signaling Peptides and Proteins metabolism, Membrane Proteins metabolism, Muscle, Smooth, Vascular growth & development, Receptors, Notch metabolism

Abstract

Background: Notch signaling in vascular smooth muscle precursors is required for smooth muscle differentiation. Jagged1 expression on endothelium activates Notch in vascular smooth muscle precursors including those of neural crest origin to initiate the formation of a smooth muscle layer in a maturing blood vessel., Methods and Results: Here, we show that Jagged1 is a direct Notch target in smooth muscle, resulting in a positive feedback loop and lateral induction that propagates a wave of smooth muscle differentiation during aortic arch artery development. In vivo, we show that Notch inhibition in cardiac neural crest impairs Jagged1 messenger RNA expression and results in deficient smooth muscle differentiation and resultant aortic arch artery defects. Ex vivo, Jagged1 ligand activates Notch in neural crest explants and results in activation of Jagged1 messenger RNA, a response that is blocked by Notch inhibition. We examine 15 evolutionary conserved regions within the Jagged1 genomic locus and identify a single Notch response element within the second intron. This element contains a functional Rbp-J binding site demonstrated by luciferase reporter and chromatin immunoprecipitation assays and is sufficient to recapitulate aortic arch artery expression of Jagged1 in transgenic mice. Loss of Jagged1 in neural crest impairs vascular smooth muscle differentiation and results in aortic arch artery defects., Conclusions: Taken together, these results provide a mechanism for lateral induction that allows for a multilayered smooth muscle wall to form around a nascent arterial endothelial tube and identify Jagged1 as a direct Notch target., (© 2011 American Heart Association, Inc.)

Published

2012

10. Cardiac neural crest orchestrates remodeling and functional maturation of mouse semilunar valves.

Author

Jain R, Engleka KA, Rentschler SL, Manderfield LJ, Li L, Yuan L, and Epstein JA

Subjects

Animals, Aortic Valve abnormalities, Aortic Valve physiopathology, Apoptosis, Endocardial Cushion Defects embryology, Endocardial Cushion Defects physiopathology, Female, Humans, Mice, Mice, Mutant Strains, Models, Cardiovascular, Neural Crest abnormalities, Neural Crest physiopathology, PAX3 Transcription Factor, Paired Box Transcription Factors deficiency, Paired Box Transcription Factors genetics, Pregnancy, Receptors, Notch genetics, Receptors, Notch physiology, Signal Transduction, Aortic Valve embryology, Neural Crest embryology

Abstract

Congenital anomalies of the aortic valve are common and are associated with progressive valvular insufficiency and/or stenosis. In addition, aneurysm, coarctation, and dissection of the ascending aorta and aortic arch are often associated conditions that complicate patient management and increase morbidity and mortality. These associated aortopathies are commonly attributed to turbulent hemodynamic flow through the malformed valve leading to focal defects in the vessel wall. However, numerous surgical and pathological studies have identified widespread cystic medial necrosis and smooth muscle apoptosis throughout the aortic arch in affected patients. Here, we provide experimental evidence for an alternative model to explain the association of aortic vessel and valvular disease. Using mice with primary and secondary cardiac neural crest deficiencies, we have shown that neural crest contribution to the outflow endocardial cushions (the precursors of the semilunar valves) is required for late gestation valvular remodeling, mesenchymal apoptosis, and proper valve architecture. Neural crest was also shown to contribute to the smooth muscle layer of the wall of the ascending aorta and aortic arch. Hence, defects of cardiac neural crest can result in functionally abnormal semilunar valves and concomitant aortic arch artery abnormalities.

Published

2011

11. Distinct enhancers at the Pax3 locus can function redundantly to regulate neural tube and neural crest expressions.

Author

Degenhardt KR, Milewski RC, Padmanabhan A, Miller M, Singh MK, Lang D, Engleka KA, Wu M, Li J, Zhou D, Antonucci N, Li L, and Epstein JA

Subjects

Animals, Animals, Genetically Modified, Embryo, Mammalian metabolism, Embryo, Nonmammalian metabolism, Mice, Mice, Transgenic, Paired Box Transcription Factors metabolism, Zebrafish embryology, Enhancer Elements, Genetic genetics, Gene Expression Regulation, Developmental, Neural Crest embryology, Neural Tube embryology, Paired Box Transcription Factors genetics

Abstract

Pax3 is a transcription factor expressed in somitic mesoderm, dorsal neural tube and pre-migratory neural crest during embryonic development. We have previously identified cis-acting enhancer elements within the proximal upstream genomic region of Pax3 that are sufficient to direct functional expression of Pax3 in neural crest. These elements direct expression of a reporter gene to pre-migratory neural crest in transgenic mice, and transgenic expression of a Pax3 cDNA using these elements is sufficient to rescue neural crest development in mice otherwise lacking endogenous Pax3. We show here that deletion of these enhancer sequences by homologous recombination is insufficient to abrogate neural crest expression of Pax3 and results in viable mice. We identify a distinct enhancer in the fourth intron that is also capable of mediating neural crest expression in transgenic mice and zebrafish. Our analysis suggests the existence of functionally redundant neural crest enhancer modules for Pax3., (Copyright 2009 Elsevier Inc. All rights reserved.)

Published

2010

12. Menin expression modulates mesenchymal cell commitment to the myogenic and osteogenic lineages.

Author

Aziz A, Miyake T, Engleka KA, Epstein JA, and McDermott JC

Subjects

Animals, Bone Morphogenetic Protein 2 pharmacology, Cell Differentiation drug effects, Cell Differentiation genetics, Cell Line, Down-Regulation drug effects, Down-Regulation genetics, Gene Deletion, Humans, Intercostal Muscles anatomy & histology, Intercostal Muscles drug effects, Mesenchymal Stem Cells drug effects, Mice, Multipotent Stem Cells cytology, Multipotent Stem Cells drug effects, Multipotent Stem Cells metabolism, Muscle Development drug effects, MyoD Protein metabolism, Myoblasts cytology, Myoblasts drug effects, Myoblasts metabolism, Organ Size drug effects, Organ Specificity drug effects, Osteoblasts cytology, Osteoblasts drug effects, Osteoblasts metabolism, Osteogenesis drug effects, Protein Binding drug effects, Proto-Oncogene Proteins genetics, Smad3 Protein metabolism, Somites cytology, Somites drug effects, Somites metabolism, Transforming Growth Factor beta1 metabolism, Cell Lineage drug effects, Mesenchymal Stem Cells cytology, Mesenchymal Stem Cells metabolism, Muscle Development genetics, Osteogenesis genetics, Proto-Oncogene Proteins metabolism

Abstract

Menin plays an established role in the differentiation of mesenchymal cells to the osteogenic lineage. Conversely, whether Menin influences the commitment of mesenschymal cells to the myogenic lineage, despite expression in the developing somite was previously unclear. We observed that Menin is down-regulated in C2C12 and C3H10T1/2 mesenchymal cells when muscle differentiation is induced. Moreover, maintenance of Menin expression by constitutive ectopic expression inhibited muscle cell differentiation. Reduction of Menin expression by siRNA technology results in precocious muscle differentiation and concomitantly attenuates BMP-2 induced osteogenesis. Reduced Menin expression antagonizes BMP-2 and TGF-beta1 mediated inhibition of myogenesis. Furthermore, Menin was found to directly interact with and potentiate the transactivation properties of Smad3 in response to TGF-beta1. Finally in concert with these observations, tissue-specific inactivation of Men1 in Pax3-expressing somite precursor cells leads to a patterning defect of rib formation and increased muscle mass in the intercostal region. These data invoke a pivotal role for Menin in the competence of mesenchymal cells to respond to TGF-beta1 and BMP-2 signals. Thus, by modulating cytokine responsiveness Menin functions to alter the balance of multipotent mesenchymal cell commitment to the osteogenic or myogenic lineages.

Published

2009

13. Persistent expression of Pax3 in the neural crest causes cleft palate and defective osteogenesis in mice.

Author

Wu M, Li J, Engleka KA, Zhou B, Lu MM, Plotkin JB, and Epstein JA

Subjects

Animals, Bone Development, DNA, Complementary metabolism, Dose-Response Relationship, Drug, Genotype, Mice, Mice, Transgenic, Models, Biological, Models, Genetic, PAX3 Transcription Factor, Paired Box Transcription Factors metabolism, Proteins genetics, RNA, Untranslated, Cleft Palate embryology, Gene Expression Regulation, Developmental, Neural Crest embryology, Osteogenesis, Paired Box Transcription Factors physiology

Abstract

Transcription factors regulate tissue patterning and cell fate determination during development; however, expression of early regulators frequently abates upon differentiation, suggesting that they may also play a role in maintaining an undifferentiated phenotype. The transcription factor paired box 3 (Pax3) is expressed by multipotent neural crest precursors and is implicated in neural crest disorders in humans such as Waardenburg syndrome. Pax3 is required for development of multiple neural crest lineages and for activation of lineage-specific programs, yet expression is generally extinguished once neural crest cells migrate from the dorsal neural tube and differentiate. Using a murine Cre-inducible system, we asked whether persistent Pax3 expression in neural crest derivatives would affect development or patterning. We found that persistent expression of Pax3 in cranial neural crest cells resulted in cleft palate, ocular defects, malformation of the sphenoid bone, and perinatal lethality. Furthermore, we demonstrated that Pax3 directly regulates expression of Sostdc1, a soluble inhibitor of bone morphogenetic protein (BMP) signaling. Persistent Pax3 expression renders the cranial crest resistant to BMP-induced osteogenesis. Thus, one mechanism by which Pax3 maintains the undifferentiated state of neural crest mesenchyme may be to block responsiveness to differentiation signals from the environment. These studies provide in vivo evidence for the importance of Pax3 downregulation during differentiation of multipotent neural crest precursors and cranial development.

Published

2008

14. Menin is required in cranial neural crest for palatogenesis and perinatal viability.

Author

Engleka KA, Wu M, Zhang M, Antonucci NB, and Epstein JA

Subjects

Abnormalities, Multiple genetics, Abnormalities, Multiple pathology, Animals, Animals, Newborn, Cells, Cultured, Cleft Palate, Humans, Mice, Mice, Transgenic, PAX3 Transcription Factor, Paired Box Transcription Factors genetics, Paired Box Transcription Factors metabolism, Proto-Oncogene Proteins genetics, Wnt1 Protein genetics, Wnt1 Protein metabolism, Fetal Mortality, Morphogenesis, Neural Crest metabolism, Palate embryology, Palate growth & development, Proto-Oncogene Proteins metabolism

Abstract

Menin is a nuclear protein encoded by a tumor suppressor gene that is mutated in humans with multiple endocrine neoplasia type 1 (MEN1). Menin functions as a component of a histone methyltransferase complex that regulates expression of target genes including the cell cycle inhibitor p27(kip1). Here, we show that menin plays a previously unappreciated and critical role in cranial neural crest. Tissue-specific inactivation of menin in Pax3- or Wnt1-expressing neural crest cells leads to perinatal death, cleft palate and other cranial bone defects, which are associated with a decrease in p27(kip1) expression. Deletion of menin in Pax3-expressing somite precursors also produces patterning defects of rib formation. Thus, menin functions in vivo during osteogenesis and is required for palatogenesis, skeletal rib formation and perinatal viability.

Published

2007

15. Somitic origin of limb muscle satellite and side population cells.

Author

Schienda J, Engleka KA, Jun S, Hansen MS, Epstein JA, Tabin CJ, Kunkel LM, and Kardon G

Subjects

Animals, Cell Lineage, Cell Movement, Cells, Cultured, Chick Embryo, Chimera, Embryo, Mammalian cytology, Embryo, Nonmammalian, Genes, Reporter, Green Fluorescent Proteins metabolism, Immunohistochemistry, Mice, Microscopy, Fluorescence, Muscles cytology, Muscles metabolism, PAX3 Transcription Factor, Paired Box Transcription Factors metabolism, Quail, Retroviridae genetics, Somites cytology, Species Specificity, Muscle Cells cytology, Satellite Cells, Skeletal Muscle cytology, Stem Cells cytology

Abstract

Repair of mature skeletal muscle is mediated by adult muscle progenitors. Satellite cells have long been recognized as playing a major role in muscle repair, whereas side population (SP) cells have more recently been identified as contributing to this process. The developmental source of these two progenitor populations has been considerably debated. We explicitly tested and quantified the contribution of embryonic somitic cells to these progenitor populations. Chick somitic cells were labeled by using replication-defective retroviruses or quail/chick chimeras, and mouse cells were labeled by crossing somite-specific, Pax3-derived Cre driver lines with a Cre-dependent reporter line. We show that the majority of, if not all, limb muscle satellite cells arise from cells expressing Pax3 specifically in the hypaxial somite and their migratory derivatives. We also find that a significant number of, but not all, limb muscle SP cells are derived from the hypaxial somite. Notably, the heterogeneity in the developmental origin of SP cells is reflected in their functional heterogeneity; somitically derived SP cells are intrinsically more myogenic than nonsomitically derived ones. Thus, we show that the somites, which supply embryonic and fetal myoblasts, are also an important source of highly myogenic adult muscle progenitors.

Published

2006

16. Insertion of Cre into the Pax3 locus creates a new allele of Splotch and identifies unexpected Pax3 derivatives.

Author

Engleka KA, Gitler AD, Zhang M, Zhou DD, High FA, and Epstein JA

Subjects

Alleles, Animals, Cell Movement, DNA-Binding Proteins metabolism, Embryo, Mammalian metabolism, Exons, Genotype, Heterozygote, Homozygote, Immunoblotting, Immunohistochemistry, In Situ Hybridization, Mice, Mice, Transgenic, Models, Genetic, Muscle, Skeletal cytology, Neurons metabolism, PAX3 Transcription Factor, Paired Box Transcription Factors, RNA, Messenger metabolism, Recombination, Genetic, Time Factors, Transcription Factors metabolism, Transcription, Genetic, beta-Galactosidase metabolism, DNA-Binding Proteins genetics, Genetic Techniques, Transcription Factors genetics

Abstract

Pax3 is a transcription factor expressed in the dorsal neural tube and somite of the developing embryo. It plays critical roles in pre-migratory neural crest cells and in myogenic precursors of skeletal muscle. Pax3-deficient Splotch embryos display neural tube and neural crest defects and lack hypaxial muscles. We have created a new allele of Splotch by replacing the first coding exon with a gene encoding Cre recombinase. This functions as a null allele and no Pax3 protein is detected in homozygous embryos. Heterozygous Pax3(Cre/+) mice display a white belly spot, as do Splotch heterozygotes. Homozygous Pax3(Cre/Cre) embryos are embryonic lethal. We have used Pax3(Cre/+) mice to fate-map Pax3 derivatives in the developing mouse. As expected, neural crest and some somitic derivatives are identified. However, we also detect previously unappreciated derivatives of Pax3-expressing precursors in the colonic epithelium of the hindgut and within the urogenital system.

Published

2005

17. Identification of a hypaxial somite enhancer element regulating Pax3 expression in migrating myoblasts and characterization of hypaxial muscle Cre transgenic mice.

Author

Brown CB, Engleka KA, Wenning J, Min Lu M, and Epstein JA

Subjects

Animals, Enhancer Elements, Genetic, Integrases metabolism, Mice, Mice, Transgenic, Models, Animal, Myoblasts physiology, PAX3 Transcription Factor, Paired Box Transcription Factors, Somites, Cell Movement, DNA-Binding Proteins biosynthesis, DNA-Binding Proteins genetics, Gene Expression Regulation, Developmental, Muscle, Skeletal embryology, Transcription Factors biosynthesis, Transcription Factors genetics

Abstract

Pax3 encodes a transcription factor that functions in the embryonic central nervous system, neural crest, and somitic mesoderm. Prior studies suggest that distinct regulatory elements regulate temporal and spatial expression of Pax3 in neural crest and mesoderm. Here, we describe a discrete enhancer element, conserved between mouse and human genomes, that directs Pax3 expression in the ventral-lateral lip of interlimb somites. These regions give rise to hypaxial musculature including limb, ventral body wall, diaphragm, and tongue muscles. Transgenic mice harboring the hypaxial muscle enhancer driving lacZ expression initiate beta-galactosidase expression at E10.0, significantly later than endogenous Pax3 expression in presomitic and segmented mesoderm. Initiation of transgene expression is not dependent on Pax3 itself, since expression is detectable in homozygous Splotch embryos. Transgenic mice expressing Cre recombinase in hypaxial myoblasts were generated and characterized. These results suggest that Pax3 is differentially regulated within the somite in both spatial and temporal domains. Hypaxial muscle Cre mice will allow for specific manipulation of gene expression in this subset of developing skeletal muscle., (Copyright (c) 2005 Wiley-Liss, Inc.)

Published

2005

18. Pax3 functions at a nodal point in melanocyte stem cell differentiation.

Author

Lang D, Lu MM, Huang L, Engleka KA, Zhang M, Chu EY, Lipner S, Skoultchi A, Millar SE, and Epstein JA

Subjects

Aging physiology, Animals, Base Sequence, Binding, Competitive, Cell Line, Cell Lineage, Cytoskeletal Proteins metabolism, Enhancer Elements, Genetic genetics, Gene Expression Regulation, Hair Follicle metabolism, Humans, Intramolecular Oxidoreductases genetics, Mice, Microphthalmia-Associated Transcription Factor, Molecular Sequence Data, PAX3 Transcription Factor, Paired Box Transcription Factors, Sequence Deletion genetics, Trans-Activators metabolism, beta Catenin, Cell Differentiation, DNA-Binding Proteins metabolism, Melanocytes cytology, Melanocytes metabolism, Stem Cells cytology, Stem Cells metabolism, Transcription Factors metabolism

Abstract

Most stem cells are not totipotent. Instead, they are partially committed but remain undifferentiated. Upon appropriate stimulation they are capable of regenerating mature cell types. Little is known about the genetic programmes that maintain the undifferentiated phenotype of lineage-restricted stem cells. Here we describe the molecular details of a nodal point in adult melanocyte stem cell differentiation in which Pax3 simultaneously functions to initiate a melanogenic cascade while acting downstream to prevent terminal differentiation. Pax3 activates expression of Mitf, a transcription factor critical for melanogenesis, while at the same time it competes with Mitf for occupancy of an enhancer required for expression of dopachrome tautomerase, an enzyme that functions in melanin synthesis. Pax3-expressing melanoblasts are thus committed but undifferentiated until Pax3-mediated repression is relieved by activated beta-catenin. Thus, a stem cell transcription factor can both determine cell fate and simultaneously maintain an undifferentiated state, leaving a cell poised to differentiate in response to external stimuli.

Published

2005

19. A potential role for the nucleolus in L1 retrotransposition.

Author

Goodier JL, Ostertag EM, Engleka KA, Seleme MC, and Kazazian HH Jr

Subjects

Cell Culture Techniques, Cell Nucleolus ultrastructure, Cloning, Molecular, Cytoplasm ultrastructure, DNA Transposable Elements, DNA-Directed RNA Polymerases genetics, Endonucleases genetics, Endonucleases metabolism, Endothelial Cells ultrastructure, Green Fluorescent Proteins analysis, Green Fluorescent Proteins genetics, Humans, Immunochemistry, Nuclear Localization Signals genetics, RNA-Directed DNA Polymerase genetics, RNA-Directed DNA Polymerase metabolism, Ribonucleoproteins genetics, Ribonucleoproteins metabolism, Umbilical Veins cytology, Viral Proteins, Cell Nucleolus chemistry, Endonucleases analysis, Long Interspersed Nucleotide Elements genetics, RNA-Directed DNA Polymerase analysis, Ribonucleoproteins analysis

Abstract

Determining the subcellular localization of the L1 ORF2 protein (ORF2p) has been impossible to date because of technical limitations in detecting either endogenous or overexpressed forms of the protein. Here we report visualization of the full-length ORF2p in cultured human cells following expression in a modified vaccinia virus/T7 RNA polymerase (MVA/T7RP) system. The MVA/T7RP system was used to ascertain subcellular localization of L1 ORF1p and ORF2p both as fusions with green fluorescent protein and by immunocytochemistry. Full-length ORF2p was predominantly cytoplasmic, while carboxy-terminal-deleted ORF2p localized additionally to the nucleolus. We mapped a functional nucleolar localization signal in ORF2p. ORF1p appeared in the cytoplasm with a speckled pattern and colocalized with ORF2p in nucleoli in a subset of cells. These findings help explain the presence of chimeras between L1s and small RNA gene sequences recently discovered in the human genome.

Published

2004

20. Mechanisms of replication-deficient vaccinia virus/T7 RNA polymerase hybrid expression: effect of T7 RNA polymerase levels and alpha-amanitin.

Author

Engleka KA, Lewis EW, and Howard BH

Subjects

Amanitins genetics, Chloramphenicol O-Acetyltransferase genetics, DNA-Directed RNA Polymerases metabolism, Defective Viruses genetics, Defective Viruses physiology, Enzyme Induction, Enzyme Inhibitors metabolism, HeLa Cells, Humans, Promoter Regions, Genetic, Vaccinia virus genetics, Vaccinia virus physiology, Viral Proteins, Virus Replication, Amanitins metabolism, DNA-Directed RNA Polymerases genetics, Defective Viruses enzymology, Gene Expression, Genetic Vectors, Vaccinia virus enzymology

Abstract

Components of the eukaryotic vaccinia virus/T7 RNA polymerase hybrid expression system were assessed using recombinant and nonrecombinant forms of modified vaccinia Ankara (MVA), a replication-deficient vaccinia virus strain. Recombinant MVA virus expressing T7 RNA polymerase (Wyatt, L. S., Moss, B., and Rozenblatt, S. (1995). Virology 210, 202-205) stimulated high levels of expression from a T7 promoter-chloramphenicol acetyltransferase (CAT) reporter. Most, but not all, of the virally induced expression was T7 RNA polymerase and T7 promoter dependent, with no viral enhancement of translation of T7 transcripts. The efficacy of supplying T7 RNA polymerase expression from nonviral sources was evaluated using a self-amplifying T7 RNA polymerase autogene or an inducible T7 RNA polymerase expression vector. The latter modes yielded CAT activity dependent on T7 RNA polymerase expression; however, expression required viral factors independent of T7 RNA polymerase and did not reach that attained using the recombinant virus. In further experiments, MVA-induced T7 RNA polymerase expression was upregulated by alpha-amanitin, an inhibitor of eukaryotic polymerases. This indicates that MVA/T7 RNA polymerase hybrid expression may be rendered still more efficient by ameliorating transcriptional interference due to an alpha-amanitin-sensitive eukaryotic factor(s).

Published

1998

21. Differential transforming abilities of non-secreted and secreted forms of human fibroblast growth factor-1.

Author

Forough R, Xi Z, MacPhee M, Friedman S, Engleka KA, Sayers T, Wiltrout RH, and Maciag T

Subjects

3T3 Cells, Amino Acid Sequence, Animals, Base Sequence, Cell Division, Fibroblast Growth Factors chemistry, Fibroblast Growth Factors metabolism, Genetic Vectors, In Vitro Techniques, Mice, Mice, Nude, Molecular Sequence Data, Neoplasm Metastasis, Neoplasms, Experimental pathology, Oligodeoxyribonucleotides chemistry, Phosphotyrosine, Protein Sorting Signals chemistry, Protein-Tyrosine Kinases metabolism, Recombinant Fusion Proteins, Structure-Activity Relationship, Transfection, Tyrosine analogs & derivatives, Tyrosine metabolism, Cell Transformation, Neoplastic drug effects, Fibroblast Growth Factors pharmacology

Abstract

Fibroblast growth factor (FGF)-1(1-154), the precursor for acidic FGF-1(21-154), is a potent angiogenic polypeptide, the structure of which lacks a signal peptide sequence for secretion. To investigate the biological significance of this structural feature, we have attempted forced secretion of FGF-1 through fusion of the entire FGF-1 coding frame with the signal peptide (sp) from the hst/KS3 gene, a secretory member of the heparin-binding growth factor family. We also studied the transforming ability of the signal-less forms of FGF-1 comprising FGF(1-154) and FGF-1(21-154). The presence of a soluble and biologically active form of FGF-1 was readily detected in the conditioned medium of NIH 3T3 cells transfected with sp-hst/KS3:FGF-1(1-154) as demonstrated by Western blot analysis and DNA synthesis assays, whereas sp-hst/KS3:FGF-1(21-154) was not detectable in conditioned medium even though the protein was detected in cellular extracts. The secreted form of sp-hst/KS3:FGF-1(1-154) stimulated the proliferation of human umbilical vein endothelial cells in vitro and was able to induce receptor-mediated tyrosine phosphorylation. Furthermore, the forced secretion of biologically active FGF-1 resulted in NIH 3T3 cell transformation as demonstrated by altered morphology in vitro, the formation of discrete colonies in soft agarose, growth under serum-free conditions, and ability to rapidly form highly vascular tumors in vivo. Interestingly, sp-hst/KS3:FGF-1(21-154) also mediated the transition to a transformed phenotype despite the inability to detect extracellular FGF-1 in the media conditioned by these NIH 3T3 cell transfectants. Although the transfection of FGF-1(21-154) yielded similar NIH 3T3 cell morphologic changes, these transfectants did not grow under serum-free conditions or yield colonies in soft agarose, and formed tumors in vivo with delayed kinetics. Furthermore, the FGF-1(1-154) NIH 3T3 cell transfectants did not exhibit morphologic changes, and this may be due to the inability of mRNA to express protein. These data suggest that although non-sp forms of FGF-1 may alter the monolayer phenotype of NIH 3T3 cells in vitro, the ability of FGF-1 to transform NIH 3T3 cells requires the function of a sp-directed secretory pathway and suggests that this pathway increases tumorigenicity in vivo.

Published

1993

22. Heat shock induces the release of fibroblast growth factor 1 from NIH 3T3 cells.

Author

Jackson A, Friedman S, Zhan X, Engleka KA, Forough R, and Maciag T

Subjects

3T3 Cells, Animals, Cell Division, Culture Media, Conditioned, Cycloheximide pharmacology, Cytosol metabolism, DNA biosynthesis, Dactinomycin pharmacology, Fibroblast Growth Factor 1 genetics, Fibroblast Growth Factor 1 metabolism, Fibroblast Growth Factor 1 pharmacology, Genes, Synthetic, Immunoblotting, Kinetics, Mice, Recombinant Proteins pharmacology, Thymidine metabolism, Transfection, Tritium, Fibroblast Growth Factor 1 biosynthesis, Hot Temperature

Abstract

Fibroblast growth factor 1 (FGF-1) is a potent angiogenic and neurotrophic factor whose structure lacks a classical signal sequence for secretion. Although the initiation of these biological activities involves the interaction between FGF-1 and cell surface receptors, the mechanism responsible for the regulation of FGF-1 secretion is unknown. We report that murine NIH 3T3 cells transfected with a synthetic gene encoding FGF-1 secrete FGF-1 into their conditioned medium in response to heat shock. The form of FGF-1 released by NIH 3T3 cells in response to increased temperature (42 degrees C, 2 hr) in vitro is not biologically active and does not associate with either heparin or the extracellular NIH 3T3 monolayer matrix. However, it was possible to derive biologically active FGF-1 from the conditioned medium of heat-shocked NIH 3T3 cell transfectants by ammonium sulfate fractionation. The form of FGF-1 exposed by ammonium sulfate fractionation is similar in size to cytosolic FGF-1 and can bind and be eluted from immobilized heparin similarly to the recombinant human FGF-1 polypeptide. Further, the release of FGF-1 by NIH 3T3 cell transfectants in response to heat shock is reduced significantly by both actinomycin D and cycloheximide. These data indicate that increased temperature may upregulate the expression of a factor responsible for the secretion of FGF-1 as a biologically inactive complex that requires an activation step to exhibit the biological activity of the extracellular polypeptide mitogen.

Published

1992

23. Inactivation of human fibroblast growth factor-1 (FGF-1) activity by interaction with copper ions involves FGF-1 dimer formation induced by copper-catalyzed oxidation.

Author

Engleka KA and Maciag T

Subjects

Base Sequence, Catalysis, Cations, Disulfides metabolism, Electrophoresis, Polyacrylamide Gel, Fibroblast Growth Factor 1 metabolism, Fibroblast Growth Factor 2 metabolism, Heparin metabolism, Humans, Molecular Sequence Data, Oxidation-Reduction, Polymers, Recombinant Proteins metabolism, Substrate Specificity, Copper metabolism, Fibroblast Growth Factor 1 antagonists & inhibitors

Abstract

Although the angiogenic proteins acidic fibroblast growth factor (FGF-1) and basic fibroblast growth factor (FGF-2) both interact with the transition metal copper, itself a putative modulator of angiogenesis, a role for copper in FGF function has not been established. Using nonreducing sodium dodecyl sulfate-polyacrylamide gel electrophoresis, we detect the complete conversion of recombinant forms of human FGF-1 monomer protein to FGF-1 homodimers after exposure to copper ions. In contrast, not all forms of bovine FGF-1 isolated from bovine brain or a recombinant preparation of human FGF-2 completely formed homodimers after exposure to copper ions under similar conditions. Since the copper-induced FGF-1 homodimers reverted to the monomer form in the presence of dithiothreitol, specific alkylation of cysteine residues by pyridylethylation prevented FGF-1 homodimer formation, and preformed FGF-1 homodimers could not be dissociated by the metal chelator EDTA, FGF-1 dimer formation appeared to result from the formation of intermolecular disulfide bonds by copper-induced oxidation of sulfhydryl residues. FGF-1 homodimers bound with similar apparent affinity as FGF-1 monomers to immobilized copper ions, both eluting at 60 mM imidazole. Both human FGF-1 monomer and dimer forms had a 6-fold higher apparent affinity for immobilized copper ions, as compared with human FGF-2, which eluted in the monomer form at 10 mM imidazole. Further, in contrast to FGF-1 monomers, which dissociate from immobilized heparin in 1.0 M NaCl, preformed FGF-1 homodimers had reduced apparent affinity for immobilized heparin and eluted at 0.4 M NaCl. In contrast, the apparent affinity of human FGF-2 for immobilized heparin was unaffected after exposure to copper ions. Heparin appeared to modulate the formation of copper-induced intermolecular disulfide bonds for FGF-1 but not FGF-2, since co-incubation of heparin and copper with FGF-1 monomers resulted in dimers and other oligomeric complexes. FGF-1 copper-induced homodimers failed to induce mitogenesis in [3H]thymidine incorporation assays, an effect which could be reversed by treatment with dithiothreitol, whereas FGF-2-induced mitogenic activity was relatively unaffected by pretreatment with copper. The differences between human FGF-1 and FGF-2 in protein-copper interactions may be due to differing free thiol content and arrangement between the two proteins. A recombinant human FGF-1 mutant containing the two cysteines conserved throughout the FGF family of proteins but lacking a cysteine residue (Cys 131) present in wild-type human FGF-1 but not human FGF-2 readily formed copper-induced dimers.(ABSTRACT TRUNCATED AT 400 WORDS)

Published

1992